{"title":"优化一种用于人类基因治疗的质粒载体中宿主细胞DNA实时定量聚合酶链反应方法。","authors":"Serge Ferro, Isabelle Fabre, Xavier Chenivesse","doi":"10.1089/hgtb.2015.155","DOIUrl":null,"url":null,"abstract":"<p><p>Gene therapy products are very complex advanced therapy medicinal products produced using different processes that require many chemical and biological reagents and production intermediates, such as producing cells. The quantification of residual impurities in gene therapy vectors is a major quality control step when these vectors are used for therapeutic purposes, whether or not they are derived from viruses. Indeed, in nonviral gene therapy products, particularly plasmid vectors used to transfer genetic material, the presence of host-cell DNA (HCDNA) from the bacterial cells used for the vector production is an important concern because of the risk of immunogenicity and insertional mutagenesis. Several methods have been developed to quantify residual HCDNA, but real-time quantitative polymerase chain reaction (qPCR) seems to be most suitable because it allows detecting traces of \"contaminating\" DNA. The French National Agency for Medicines and Health Products Safety (ANSM) ensures the quality and safety of gene transfer medicinal products and must be able to quantify, in its own laboratories, the amount of HCDNA present in plasmid vector batches. Therefore, we developed and validated a qPCR method to quantify at the femtogram level the presence of Escherichia coli residual DNA in plasmid vectors. This approach uses the capillary-based LightCycler 1.5 System (Roche) with SYBR Green I, a primer pair against the E. coli 23S ribosomal RNA gene and different concentrations of a linearized plasmid that contains the 23S target sequence, as standard. This qPCR method is linear on an 8-decade logarithmic scale, accurate, reproducible, and sensitive (quantification of up to 10 copies of 23S target sequence per reaction, or 1.4 E. coli genome, or 7 fg of bacterial DNA). This technique allows ensuring that batches of plasmid vectors to be used in clinical trials comply with the specifications on HCDNA content.</p>","PeriodicalId":13126,"journal":{"name":"Human Gene Therapy Methods","volume":"27 4","pages":"159-70"},"PeriodicalIF":0.0000,"publicationDate":"2016-08-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://sci-hub-pdf.com/10.1089/hgtb.2015.155","citationCount":"3","resultStr":"{\"title\":\"Optimizing a Method for the Quantification by Quantitative Real-Time Polymerase Chain Reaction of Host Cell DNA in Plasmid Vector Batches Used in Human Gene Therapy.\",\"authors\":\"Serge Ferro, Isabelle Fabre, Xavier Chenivesse\",\"doi\":\"10.1089/hgtb.2015.155\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<p><p>Gene therapy products are very complex advanced therapy medicinal products produced using different processes that require many chemical and biological reagents and production intermediates, such as producing cells. 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引用次数: 3
摘要
基因治疗产品是非常复杂的先进治疗药物产品,使用不同的工艺生产,需要许多化学和生物试剂以及生产中间体,例如生产细胞。当这些载体用于治疗目的时,无论它们是否来自病毒,对基因治疗载体中残留杂质的定量是一个主要的质量控制步骤。事实上,在非病毒基因治疗产品中,特别是用于转移遗传物质的质粒载体中,来自用于载体生产的细菌细胞的宿主细胞DNA (HCDNA)的存在是一个重要的问题,因为存在免疫原性和插入突变的风险。已经开发了几种方法来量化残留的HCDNA,但实时定量聚合酶链反应(qPCR)似乎是最合适的,因为它可以检测到“污染”DNA的痕迹。法国国家药品和健康产品安全局(ANSM)确保基因转移药品的质量和安全性,并且必须能够在其自己的实验室中量化质粒载体批次中存在的HCDNA的数量。因此,我们开发并验证了一种qPCR方法,用于在飞图水平上量化质粒载体中大肠杆菌残留DNA的存在。该方法使用基于毛细管的LightCycler 1.5系统(Roche),带有SYBR Green I(针对大肠杆菌23S核糖体RNA基因的引物对)和不同浓度的含有23S靶序列的线性化质粒作为标准。这种qPCR方法在80年的对数尺度上是线性的,准确,可重复,敏感(每次反应定量多达10个拷贝23S目标序列,或1.4个大肠杆菌基因组,或7 fg细菌DNA)。该技术可确保用于临床试验的质粒载体批次符合HCDNA含量规范。
Optimizing a Method for the Quantification by Quantitative Real-Time Polymerase Chain Reaction of Host Cell DNA in Plasmid Vector Batches Used in Human Gene Therapy.
Gene therapy products are very complex advanced therapy medicinal products produced using different processes that require many chemical and biological reagents and production intermediates, such as producing cells. The quantification of residual impurities in gene therapy vectors is a major quality control step when these vectors are used for therapeutic purposes, whether or not they are derived from viruses. Indeed, in nonviral gene therapy products, particularly plasmid vectors used to transfer genetic material, the presence of host-cell DNA (HCDNA) from the bacterial cells used for the vector production is an important concern because of the risk of immunogenicity and insertional mutagenesis. Several methods have been developed to quantify residual HCDNA, but real-time quantitative polymerase chain reaction (qPCR) seems to be most suitable because it allows detecting traces of "contaminating" DNA. The French National Agency for Medicines and Health Products Safety (ANSM) ensures the quality and safety of gene transfer medicinal products and must be able to quantify, in its own laboratories, the amount of HCDNA present in plasmid vector batches. Therefore, we developed and validated a qPCR method to quantify at the femtogram level the presence of Escherichia coli residual DNA in plasmid vectors. This approach uses the capillary-based LightCycler 1.5 System (Roche) with SYBR Green I, a primer pair against the E. coli 23S ribosomal RNA gene and different concentrations of a linearized plasmid that contains the 23S target sequence, as standard. This qPCR method is linear on an 8-decade logarithmic scale, accurate, reproducible, and sensitive (quantification of up to 10 copies of 23S target sequence per reaction, or 1.4 E. coli genome, or 7 fg of bacterial DNA). This technique allows ensuring that batches of plasmid vectors to be used in clinical trials comply with the specifications on HCDNA content.
期刊介绍:
Human Gene Therapy is the premier, multidisciplinary journal covering all aspects of gene therapy. The Journal publishes in-depth coverage of DNA, RNA, and cell therapies by delivering the latest breakthroughs in research and technologies. Human Gene Therapy provides a central forum for scientific and clinical information, including ethical, legal, regulatory, social, and commercial issues, which enables the advancement and progress of therapeutic procedures leading to improved patient outcomes, and ultimately, to curing diseases.
The Journal is divided into three parts. Human Gene Therapy, the flagship, is published 12 times per year. HGT Methods, a bimonthly journal, focuses on the applications of gene therapy to product testing and development. HGT Clinical Development, a quarterly journal, serves as a venue for publishing data relevant to the regulatory review and commercial development of cell and gene therapy products.
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